For the in vitro studies, CF airway epithelial cells (IB3-1, ΔF508/W1282X, American Type Culture Collection (ATCC), Manassas, VA) were cultured and maintained in LHC-8 medium containing 10% FBS, 100 units/mL penicillin, and 100 μg/mL streptomycin. WLBU-2 (25μM) was added to the media with qRT-PCR measurement of TNF-α and IL-1β transcripts after 20, 30, and 60min. IB3-1 cells were used for flow cytometry ¹² and measurement of proinflammatory cytokine activity. Transfected cells containing a wild-type or NFκB mutant-IL-8 promoter gene ¹³ were treated with WLBU-2 followed by measurement of IL-8 reporter activity.

These studies used CF IB3-1 (ΔF508/W1282X) cells, transiently transfected with α 5' firefly luciferase gene (Clontech Laboratories, Inc, Mountain View, CA) flanking a wild type- or NFκB mutant-IL-8 promoter, using Lipofectamine 2000 (Invitrogen, Carlsbad, CA) for 24h as previously described ^{13, 14} . The CAP LL-37 (25μM) or the eCAP WLBU-2 (25μM) was added to the media for 30min-4h. The Dual-Luciferase ^® Reporter (DLRTM) Assay System (Clontech Laboratories, Inc, Mountain View, CA) was used to measure IL-8 reporter activity in IB3-1 cells. Renilla luciferase (Clontech Laboratories, Inc, Mountain View, CA) was used as an internal control to normalize changes in IL-8 promoter-driven firefly luciferase activity across the samples.

IB3-1 cells were incubated overnight at 37°C with LPS-Alexa Fluor 488 (Invitrogen, Carlsbad, CA) and Lipofectamine 2000. PBS or WLBU-2 (25µM) was added to the flask for 24h. After the addition of Cell Dissociation Buffer (Invitrogen, Carlsbad, CA), cells were collected, centrifuged, and rinsed with PBS. Finally, cells were treated with FIX & PERM (Invitrogen, Carlsbad, CA) per the manufacturer’s directions. Flow cytometry was done on a BD FACS can flow cytometer and data were analyzed using CellQuest.

This protocol was approved by the institutional Animal Care and Use Committee (ACUC). Animals used in this study were followed for 1–5 days (4 animals per cage) in approved satellite housing to allow close observation from the beginning to end of each experiment. Feeding practices, light cycle, and temperature and humidity, and cage and room cleaning procedures were identical to those of this institution’s central animal facility in accordance with ACUC recommendations. Animals were studied in four groups of four animals per experiment. The groups consisted of a) control C57/BL6 wild-type mice; b) C57/BL6 wild-type mice receiving bacteria (positive control); c) the eCAP WLBU-2 or the CAP LL-37 (test agents); or d) the combination of bacteria and WLBU-2 or LL-37. Animals in the experimental groups received the test agents, while control animals received sterile phosphate-buffered saline via the trachea using the posterior pharyngeal approach. These studies were carried out in the presence or absence of a proinflammatory stimulus (bacterial exposure).

Mice were anesthetized using a vaporizer set to deliver a mixture of 3% isoflurane and oxygen in preparation for the instillation of control or test agents into the respiratory tree. Complete anesthesia was determined by visual confirmation of a slowed respiration rate and the animal’s response to other clinical tests such as leg withdrawal and tail pinch. Animals were weighed prior to the procedure. The method is based on a published study ¹⁵ . Once anesthetized, the tongue was gently extruded using padded forceps and the control and/or test agents (volume 50µL) were pipetted into the posterior section of the oral cavity. The positive control was 1) P. aeruginosa (ATCC type strain, 1×10 ⁶ cfu/mL); the negative control was PBS. The test agents were the host-derived CAP LL-37 or the engineered CAP WLBU-2 (dose 1mg/kg). Following aspiration of the test agent, 100% O ₂ was given until the animal awakened. Animals were then placed into a 37°C chamber until completely recovered.

Intraperitoneal PA infection in age (8 weeks) and sex-matched C57BL/6 mice was established ¹⁶ followed by WLBU-2 (4mg/kg), LL-37 (4mg/kg), or PBS treatment ⁵ , followed by collection at 24h of bronchoalveolar lavage (BAL) samples and lung tissue for bacterial culture on trypticase soy agar plates, quantitative RT-PCR, ELISA, and microscopy ¹² . Mice were anesthetized with 3% isoflurane before and during treatment. After 24h, mice were sacrificed for sample collection.

At the endpoint of the experiments mice were anesthetized using a vaporizer set to deliver a mixture of 3% isoflurane and oxygen and weighed. Once completely anesthetized, animals were euthanized by cervical dislocation followed by collection of BAL samples from within an exposed thorax using sterile phosphate-buffered saline (PBS) through a cannula inserted in the trachea. BAL samples were used for protein analysis as well as leukocyte differentiation. Lungs were excised and then stored in buffers or preservatives for protein analysis or histologic examination.

Mouse lungs were homogenized in TRIzol (Invitrogen, Carlsbad, CA) and processed for isolation of total RNA according to the manufacturer's instructions. The Super Script III First-Strand Synthesis System (Invitrogen, Carlsbad, CA) was used to catalyze the reverse transcription reaction from 1µg of total RNA. Quantitative RT-PCR (qRT-PCR) was performed using TaqMan Gene Expression Master Mix and TaqMan Gene Expression Assays (Applied Biosystems, Foster City, CA) for GAPDH (control reagent), IL-1β, and TNF-α (4352932, Mm01336189_m1, Mm99999068_m1, respectively). The qRT-PCR reactions were amplified using an ABI PRISM 7700 Sequence Detection System. Relative gene expression was determined using ∆∆Ct calculations.

ELISA kits for IL-1β and IL-6 were obtained from R&D Systems (Minneapolis, MN). The manufacturer’s protocol was followed for the detection of each cytokine in 10µL of BAL fluid as well as in standardized samples provided in the kit. SoftMax Pro (Molecular Devices, Sunnyvale, CA) was used to read the 96-well plates in a Molecular Devices VersaMax microplate reader. A plot of the standardized samples was used to calculate cytokine expression in the BAL samples. For histologic examination, lungs were fixed overnight in 4% paraformaldehyde at 4°C and subsequently embedded in paraffin. Tissue sections (5µm thickness) were deparaffinized and rehydrated with xylenes and a series of decreasing ethanol concentrations, respectively. Hematoxylin and eosin were used to stain the sections prior to microscopic examination.

IB3-1 cells were used to examine proinflammatory cytokine effects after WLBU-2 exposure. IL-8 promoter activity was significantly increased compared to control in both WLBU-2-exposed IB3-1 cells after 4h (mean±SD 1.14±0.0004 vs. 0.67±0.0002, p<0.005, Figure 1) and LL-37-exposed cells (mean±SD 1.04±0.0006 vs. 0.67±0.0002, Figure 1). WLBU-2-exposed cells showed significantly less IL-8 promoter activity compared to LL-37-exposed cells ( p<0.005). IB3-1 cells with an NFκB mutant IL-8 promoter exposed to either peptide showed minimal reporter activity at 4h ( Figure 1), suggesting that both WLBU-2 and LL-37 influence IL-8 secretion through NFκB. Exposure to either WLBU-2 (25μM) or LL-37 (25μM) for 30min ( Figure 2) resulted in increased transcript levels of IL-1β (mean±SD fold-change WLBU-2 1.59±0.12; LL-37 1.47±0.12, p<0.005) and TNF-α (mean±SD fold-change WLBU-2 5.74±1.83; LL-37 4.11±1.07, p<0.005) compared to control and decreased by 60min toward baseline (see raw data file).

Using equimolar (25μM) peptide concentrations in LPS-stimulated cells, WLBU-2 showed less LPS-induced IL-8 reporter activity compared to LL-37 after 4h (mean±SD 1.82±0.0034 vs. 2.93±0.0009, p<0.005, Figure 3). By flow cytometry, WLBU-2-exposed cells showed 91% uptake of fluorescently labeled LPS after 24h compared to 75% of control cells. These results suggest that WLBU-2 induces a protective inflammatory response through interaction with LPS (T. Mietzner, unpublished observation) and exhibits an initial protective effect against epithelial inflammatory challenges.

WLBU-2 treatment of animals (n=5/group) with intraperitoneal PA infection showed more IL-1β suppression compared to LL-37 (mean±SD fold-change 37.6±9.7 vs. 105.9±30.9, p<0.005, Figure 4). There was no effect on TNF-α (data not shown). Consistent with prior efficacy studies comparing the bactericidal activities of WLBU-2 and LL-37 ^{5, 6} , bacterial cultures of lung homogenates from WLBU-2-treated animals showed no growth compared to those given LL-37 after 24h (0 cfu/mL vs. 5800 cfu/mL).